ALBERT — All Library Books, journals and Electronic Records Telegrafenberg

1

Electronic Resource

Characterization of two new members of the pregnancy-specific .beta.1-glycoprotein family from the myeloid cell line KG-1 and suggestion of two distinct classes of transcription unit (1990)

Barnett, Thomas R. ; Pickle, William ; Elting, James J.

s.l. : American Chemical Society

Biochemistry 29 (1990), S. 10213-10218

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ISSN: 1520-4995

Source: ACS Legacy Archives

Topics: Biology , Chemistry and Pharmacology

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1021/bi00496a009

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2

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DNA sequence organization in the genomes of five marine invertebrates (1975)

Goldberg, Robert B. ; Crain, William R. ; Ruderman, Joan V. ; [et al.]

Springer

Chromosoma 51 (1975), S. 225-251

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ISSN: 1432-0886

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Abstract The arrangement of repetitive and non-repetitive sequence was studied in the genomic DNA of the oyster (Crassostrea virginica), the surf clam (Spisula solidissima), the horseshoe crab (Limulus polyphemus), a nemertean worm (Cerebratulus lacteus) and a jellyfish (Aurelia aurita). Except for the jellyfish these animals belong to the protostomial branch of animal evolution, for which little information regarding DNA sequence organization has previously been available. The reassociation kinetics of short (250–300 nucleotide) and long (2,000–3,000 nucleotide) DNA fragments was studied by the hydroxyapatite method. It was shown that in each case a major fraction of the DNA consists of single copy sequences less than about 3,000 nucleotides in length, interspersed with short repetitive sequences. The lengths of the repetitive sequences were estimated by optical hyperchromicity and S1 nuclease measurements made on renaturation products. All the genomes studied include a prominent fraction of interspersed repetitive sequences about 300 nucleotides in length, as well as longer repetitive sequence regions.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00284817

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3

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Nontranscribed spacers in Drosophila ribosomal DNA (1981)

Rae, Peter M. M. ; Barnett, Thomas ; Murtif, Vicki L.

Springer

Chromosoma 82 (1981), S. 637-655

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ISSN: 1432-0886

Source: Springer Online Journal Archives 1860-2000

Topics: Biology , Medicine

Notes: Abstract Ribosomal DNA nontranscribed spacers in Drosophila virilis DNA have been examined in some detail by restriction site analysis of cloned segments of rDNA, nucleic acid hybridizations involving unfractionated rDNA, and base composition estimates. The overall G+C content of the spacer is 27–28%; this compares with 39% for rDNA as a whole, 40% for main band DNA, and 26% for the D. virilis satellites. Much of the spacer is comprised of 0.25 kb repeats revealed by digestion with Msp I, Fnu DII or Rsd I, which terminate very near the beginning of the template for the ribosomal RNA precursor. The spacers are heterogeneous in length among rDNA repeats, and this is largely accounted for by variation among rDNA units in the number of 0.25 kb elements per spacer. Despite its high A+T content and the repetitive nature of much of the spacer, and the proximity of rDNA and heterochromatin in Drosophila, pyrimidine tract analysis gave no indication of relatedness between the spacer and satellite DNA sequences. Species of Drosophila closely related to D. virilis have rDNA spacers that are homologous with those in D. virilis to the extent that hybridization of a cloned spacer segment of D. virilis rDNA to various DNA is comparable with hybridization to homologous DNA, and distributions of restriction enzyme cleavage sites are very similar (but not identical) among spacers of the various species. There is spacer length heterogeneity in the rDNA of all species, and each species has a unique major rDNA spacer length. Judging from Southern blot hybridization, D. hydei rDNA spacers have 20–30% sequence homology with D. virilis rDNA spacers, and a repetitive component is similarly sensitive to Msp I and Fnu DII digestion, D. melanogaster rDNA spacers have little or no homology with counterparts in D. virilis rDNA, despite a similar content of 0.25 kb repetitive elements. In contrast, sequences in rDNA that encode 18S and 28S ribosomal RNA have been highly conserved during the divergence of Drosophila species; this is inferred from interspecific hybridizations involving ribosomal RNA and a comparison of distributions of restriction enzyme cleavage sites in rDNA.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00285773

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4

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Heat shock induced proteins in plant cells (1979)

Barnett, Thomas ; Altschuler, Mitchell ; McDaniel, Carl N. ; [et al.]

Chichester [u.a.] : Wiley-Blackwell

Developmental Genetics 1 (1979), S. 331-340

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ISSN: 0192-253X

Keywords: heat-shock ; proteins ; tobacco ; soybean ; Life and Medical Sciences ; Genetics

Source: Wiley InterScience Backfile Collection 1832-2000

Topics: Biology

Notes: Tobacco (Nicotiana tabacum) and soybean (Glycine max) tissue culture cells were exposed to a heat shock and protein synthesis studied by SDS-polyacrylamide gel electrophoresis after labeling with radioactive amino acids. A new pattern of protein synthesis is observed in heat-shocked cells compared to that in control cells. About 12 protein bands, some newly appearing, others synthesized in greatly increased quantities in heat-shock cells, are seen. Several of the heat-shock proteins (HSPs) in both tobacco and soybean are similar in size. One of the HSPs in soybean (76K) shares peptide homology with its presumptive 25°C counterpart, indicating that the synthesis of at least some HSPs may not be due to activation of new genes. The optimum temperature for maximal induction of most HSPs is 39-40°C. Total protein synthesis decreases as heat-shock temperature is increased and is barely detectable at 45°C. The heat-shock response is maintained for a relatively short time in tobacco cells. After 3 hr at 39°C, a decrease is seen in the synthesis of the HSPs, and after 4 hr practically no HSPs are synthesized. After exposure to 39°C for 1 hr, followed by a return of tobacco cells to 26°C, recovery to the control pattern of synthesis requires greater than 6 hours. These results indicate that cells of flowering plants exhibit a heat-shock response similar to that observed in animal cells.

Additional Material: 7 Ill.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1002/dvg.1020010406

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5

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Influence of basement structures on in situ stresses over the Surat Basin, southeast Queensland (2015)

Samuel Brooke-Barnett, Thomas Flottmann, Pijush K. Paul, Seth Busetti, Peter Hennings, Ray Reid, Gideon Rosenbaum

Wiley

In: Journal of Geophysical Research JGR - Solid Earth

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Publication Date: 2015-06-24

Description: The Jurassic to Cretaceous sedimentary rocks of the Surat Basin in southeast Queensland host a significant volume of coal seam gas resources. Consequently, knowledge of the in situ stress is important for coal permeability enhancement and wellbore stability. Using wireline log data and direct stress measurements, we have calculated stress orientations from 36 wells, and stress magnitudes from 7 wells across the Surat Basin. Our results reveal a relationship between high tectonic stress and proximity to structures within the underlying “basement” rocks. The influence of tectonic stresses is diminished with depth in areas with thicker sedimentary cover that are relatively far from the basement structures. We suggest that this relationship is due to the redistribution of in situ stresses around areas where basement is shallower, and where basement structures, such as the Leichhardt-Burunga Fault System, are present. This behaviour is explained by a lower rigidity in the thickest basin cover, which reduces the ability to maintain higher tectonic stress. Over the entire Surat Basin, a significant amount of variability in in situ stress orientation is observed. The authors attribute this stress variability to complex plate boundary interactions on the northern and eastern margins of the Indo-Australian plate.

Print ISSN: 0148-0227

Topics: Geosciences , Physics

Published by Wiley on behalf of American Geophysical Union (AGU).

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Multiphoton Photochemistry of Red Fluorescent Proteins in Solution and Live Cells (2014)

Mikhail Drobizhev, Caleb Stoltzfus, Igor Topol, Jack Collins, Geoffrey Wicks, Alexander Mikhaylov, Lauren Barnett, Thomas E. Hughes and Aleksander Rebane

American Chemical Society (ACS)

In: Journal of Physical Chemistry B

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Publication Date: 2014-07-25

Description: The Journal of Physical Chemistry B DOI: 10.1021/jp502477c

Electronic ISSN: 1520-5207

Topics: Chemistry and Pharmacology , Physics

Published by American Chemical Society (ACS)

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7

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Nontranscribed spacers in Drosophila ribosomal DNA (1981)

Rae, Peter M. M. ; Barnett, Thomas ; Murtif, Vicki L.

Springer

In: Chromosoma. 1981; 82(5): 637-655. Published 1981 May 01. doi: 10.1007/bf00285773.

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Publication Date: 1981-05-01

Print ISSN: 0009-5915

Electronic ISSN: 1432-0886

Topics: Biology , Medicine

Published by Springer

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Solubility limits and LaGaO3 compatibility in the LaO1.5-GaO1.5-NiO ternary system (2017)

Patrick K. Duffy, Rachel A. Beal, Carys E. Layton, Scott A. Barnett, Thomas O. Mason

Wiley

In: Journal of the American Ceramic Society

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Publication Date: 2017-01-20

Description: Phase compatibility and solubility limits in the LaO 1.5 -GaO 1.5 -NiO system at 1400°C were measured using phase analysis and disappearing phase methods, focusing on compatibility of LaGaO 3 with NiO and La n +1 Ni n O 3 n +1 Ruddlesden-Popper phases. For the first time, it was observed that, similar to La 4 Ni 3 O 10 , the incorporation of gallium stabilized La 3 Ni 2 O 7 over a narrow composition range. The compositional limits of stability involving LaGaO 3 were determined in detail, and the full quasiternary diagram is presented as a best estimation that is consistent with the observations of this study. LaGaO 3 showed compatibility with NiO, with gallium and nickel substituting for each other in both phases. The lowest attainable amount of nickel in LaGaO 3 in equilibrium with gallium-saturated NiO was measured to be around 7% nickel on gallium sites. Of the Ruddlesden-Popper phases, only La 4 Ni 3 O 10 showed compatibility with LaGaO 3 , with the two-phase region spanning between ~40%-55% gallium on nickel sites in La 4 Ni 3 O 10 and ~20%-50% nickel on gallium sites in LaGaO 3 . The electrical conductivity of La 4 (Ni 1− x Ga x ) 3 O 10 was also measured, and found to decrease monotonically with the addition of gallium. Implications relating to fabrication of solid oxide fuel cells with Sr- and Mg-doped LaGaO 3 electrolytes are discussed.

Print ISSN: 0002-7820

Electronic ISSN: 1551-2916

Topics: Mechanical Engineering, Materials Science, Production Engineering, Mining and Metallurgy, Traffic Engineering, Precision Mechanics

Published by Wiley

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The Effect of Soluble P-Selectin in Coagulation (2008)

Korakas, Ingrid ; Guillen, Darlene ; Martin, Erika ; [et al.]

American Society of Hematology

In: Blood. 2008; 112(11): 4106-4106. Published 2008 Nov 16. doi: 10.1182/blood.v112.11.4106.4106.

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Publication Date: 2008-11-16

Description: P-selectin, a member of the selectin family, is a vascular cell adhesion molecule. It is expressed and stored in alpha granules of platelets and in Weibel-Palade bodies of endothelial cells, and upon activation, P-selectin is translocated/transferred to the membrane surface. A key function of the P-selectin is to mediate leukocyte, lymphocyte and platelet interactions in inflammation and possibly in the thrombus formation. A soluble variant, S-Psel, comprising the extracellular domain of P-selectin, has been identified in healthy individuals, but is markedly elevated in patient with vascular disorders. Recent work on S-Psel suggested that S-Psel may play a role in hemostasis/coagulation through the generation of procoagulant TF-bearing microparticles (MP), and therefore, has potential in treating patients with the bleeding disorders, like hemophilia. The aim of this study is to verify studies reporting that S-Psel exhibits in vitro and in vivo pro-coagulant activity. S-Psel and S-Psel-Fc (IgG) fusion were purchased commercially or prepared at Novo Nordisk Research US (NNRUS) and their biological activity was verified by P-selectin/Pselectin glycoprotein ligand-1(PSGL-1) interaction in vitro. The clotting times of human whole blood and plasma treated with S-Psel or S-Psel-Fc, or with an irrelevant human IgG control protein, were measured by thromboelastography and aggregometry respectively. After up to 8 hours of incubation with S-Psel and S-Psel-Fc at a concentration of 15ug/ml, we found no significant difference between samples treated with S-Psel, S-Psel-Fc and the IgG controls. The ability of S-Psel to generate TF-bearing microparticles in human whole blood was examined in a FXa substrate cleavage assay; however, no significant difference in cleavage was observed. Finally, we evaluated S-Psel in vivo. Hemophilia A mice were injected with recombinant mouse S-Psel-IgG or S-Psel-Fc (IgG) at the concentration of 1.2 mg/Kg body weight and human IgG was used as control. As suggested from published results, the effect of S-Psel was determined 6 h after the treatment. Contrary to previous reports, the results revealed no significant difference in bleed time and blood loss between the experimental and control group. In conclusion, we were unable to demonstrate the procoagulant activity of S-Psel in our laboratory either in vitro or in vivo.

Print ISSN: 0006-4971

Electronic ISSN: 1528-0020

Topics: Biology , Medicine

Published by American Society of Hematology

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